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CN105267240B - The purposes of the excretion body of source for mesenchymal stem cells - Google Patents

The purposes of the excretion body of source for mesenchymal stem cells Download PDF

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CN105267240B
CN105267240B CN201410781765.3A CN201410781765A CN105267240B CN 105267240 B CN105267240 B CN 105267240B CN 201410781765 A CN201410781765 A CN 201410781765A CN 105267240 B CN105267240 B CN 105267240B
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exosome
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damage
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CN105267240A (en
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张晓敏
李筱荣
苏畅
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TIANJIN MEDICAL UNIVERSITY EYE HOSPITAL
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TIANJIN MEDICAL UNIVERSITY EYE HOSPITAL
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Abstract

The present invention relates to the purposes of the excretion body of source for mesenchymal stem cells, specifically: application of the excretion body (exosome) of source for mesenchymal stem cells in preparation treatment ophthalmology disease drug.The ophthalmology disease includes retinal damage caused by uveitis, detachment of retina, retinosis, a variety of causes and inflammation.It is demonstrated experimentally that exosome has neurotrophy and immunosuppressive action, retinal damage caused by a variety of causes can be mitigated, mitigate inflammatory reaction, so as to improve retinal function, open up new way for clinical treatment ophthalmology disease.

Description

The purposes of the excretion body of source for mesenchymal stem cells
Technical field
The invention belongs to medicament research and development, cell biologies, molecular biology field.It is related to mescenchymal stem cell Active constituent excretion body (exosome) is in preparation treatment ophthalmology disease drug in (mesenchymal stem cell, MSC) Application.
Background technique
Mescenchymal stem cell (MSC) is currently known to play a role in treating various tissue damages and immunity disease. We also turn out that MSC is including After Retinal Ischemia-reperfusion Injury, diabetic retinopathy, uveoretinitis, retinal degeneration Property and a variety of ophthalmology disease models such as retinal damage in there is therapeutic effect.MSC can be from several adult tissues (including bone Marrow, adipose tissue, Cord blood) separation, and expand in vitro.However, there is shifting since MSC cell products storage and transport are difficult Plant that survival rate is low and long-term clinical application there may be the deficiencies of tumorigenesis hidden danger that its clinical application is restricted, therefore, seek Look for it is a kind of it is easy to operate, safely and effectively the acellular therapy based on MSC seems particularly significant.
Excretion body (exosome) is a kind of film property vesica for extracting from cell culture medium supernatant, contains its derived cell After birth and cytoplasmic protein ingredient, therefore it is easier to merge with the after birth of adjacent cells, so by the after birth of cell and Cytoplasmic protein passes to another cell, carries out information transmitting in different iuntercellulars.In addition, many cells include what MSC secreted Excretion body also includes can be in the RNA (mRNA and microRNAs) that iuntercellular is shifted, by shifting in intercellular levels Mode activates target cell to generate some column biological effects.Therefore, excretion body has highly important work in cell micro-environment With.
The researchs such as Bruno discovery MSC can secrete a kind of non-solubility microvesicle of 80nm-1 μm of size of diameter, it is to acute kidney Damage has repair.These microvesicles separated from MSC supernatant can promote renal cells in vitro Proliferation and anti-apoptotic, are injected into acute kidney injury animal model body after being marked, it is possible to find microvesicle is damaged in kidney in 6h Assembled traumatic part position.2010, Singapore scholar had found that the exosome of MSC cell secretion can reduce cardiac perfusion Damage.The exosome diameter about 50-100nm of MSC secretion, has found after co-immunoprecipitation, exosome expression CD81, CD9, The albumen such as Alix.Exosome is injected mouse cardiac muscle ischemia/reperfusion model by them, and discovery can reduce infarct size.Cause This, the exosome of MSC source has the function of cardioprotection.The exosome of the MSC secretion of Cord Blood-Derived is also used for alleviating Liver fibrosis.Studies have shown that Cord blood MSC-exosome can reduce the fibrosis of liver surface, it is allowed to restore softer quality, Alleviate liver inflammation.In the Liver Fibrosis Model of CCL4 induction, 1,3 Collagen Type VIs deposition can be reduced.These are studies have shown that MSC Information transmitting can be carried out in iuntercellular by paracrine excretion body to repair damaged tissues by certain mechanism, this Paracrine mechanism is that important foundation has been established in the acellular treatment based on MSC.
The object of the present invention is to provide a kind of excretion bodies (exosome) of source for mesenchymal stem cells to treat ophthalmology in preparation New application in disease medicament opens up new way for clinical treatment ophthalmology disease.
Summary of the invention
The object of the present invention is to provide a kind of excretion bodies (exosome) of source for mesenchymal stem cells to treat ophthalmology in preparation Application in disease medicament.
The technical solution adopted by the present invention are as follows:
The present invention provides a kind of excretion bodies (exosome) of source for mesenchymal stem cells to treat ophthalmology disease medicine in preparation Application in object.
The mescenchymal stem cell is the mescenchymal stem cell of the mescenchymal stem cell in people's umbilical cord source, Human plactnta source Or the mescenchymal stem cell that people is adipose-derived.Preferably, the mescenchymal stem cell is that the mesenchyma in people's umbilical cord source is dry thin The mescenchymal stem cell in born of the same parents or Human plactnta source.It is highly preferred that the mescenchymal stem cell is the mesenchyma in people's umbilical cord source Stem cell.
The ophthalmology disease includes retina caused by uveitis, detachment of retina, retinosis, a variety of causes Damage and inflammation.
The excretion body for the source for mesenchymal stem cells that the present invention refers to has the feature that diameter is about 50-100nm, tool There are lipid film, the inhereditary materials such as interior package protein and mRNA, microRNA.(2) contain CD9, CD81, Alix through analysis of protein Equal protein moleculars, and with mescenchymal stem cell marker consistent protein molecular CD44, CD29.
The excretion body (exosome) for the source for mesenchymal stem cells that the present invention refers to, the method system by including the following steps It is standby to obtain:
(1) mescenchymal stem cell is separately cultured:
According to source for mesenchymal stem cells difference, mode is separately cultured using different:
1. human umbilical cord mesenchymal stem cells are separately cultured: the fresh umbilical cord of sterile newborn is taken, through phosphate buffer (PBS) after repeated flushing, it is cut into the tissue block of diameter about 1-2mm;After 2 Collagenase Types and pancreatin digestion successively, by supernatant Centrifugation, takes cell precipitation to be put into culture bottle, using containing 10% fetal calf serum DMEM/F12 culture medium, 5%CO2, 37 DEG C of saturations it is wet Degree culture;Non-adherent cell is removed, 0.25% trypsin digestion carries out secondary culture after attached cell 80% is merged;
2. Human plactnta mescenchymal stem cell is separately cultured: the tissue of clip placental villi film surface 1-2cm thickness is cut into 1- The fragment of 2mm is rinsed with phosphate buffer to colourless, small with Dispase II type enzyme and 4 Collagenase Types, 37 DEG C of water-baths digestion 1 When, it is stood after oscillation, liquid is divided into three layers naturally, draws middle layer suspension in centrifuge tube, and phosphate buffer is added and mixes After be centrifuged, abandon supernatant, take cell precipitation to be put into culture bottle, using contain 10% fetal calf serum DMEM culture medium, 5%CO2, 37 DEG C it is full With humidity culture;Non-adherent cell is removed, 0.25% trypsin digestion carries out secondary culture after attached cell 80% is merged;
3. human adipose mesenchymal stem cells are separately cultured: sterile aspirating adipose extract is rinsed with phosphate buffer For several times.Remove liposuction procedures in drug and haemocyte used, with 37 DEG C of 1 Collagenase Type digest 1 hour, or stirring;After centrifugation Upper-layer fat is discarded, mixes, with 200 mesh net filtrations, cell suspension obtained is centrifuged, cell precipitation phosphate-buffered Liquid washing is suspended with the α-MEM culture solution of 10% fetal calf serum, is transferred in culture bottle, 5%CO2, 37 DEG C of saturated humidity trainings It supports;0.25% trypsin digestion carries out secondary culture after attached cell 80% is merged;
(2) collection of mescenchymal stem cell conditioned medium: the mesenchymal stem cell serum-free culture 48h in 3-5 generation is taken;It receives Collect culture supernatant;0.22 μm of non-velum filteration obtains mescenchymal stem cell conditioned medium;
(3) it includes: 4 DEG C of mescenchymal stem cell conditioned medium for collecting filtering, 1000g centrifugation that exosome, which is isolated and purified, 10min collects supernatant;4 DEG C of the supernatant of collection, 2000g are centrifuged 20min, collect supernatant;4 DEG C of the supernatant of collection, 10000g It is centrifuged 30min, collects supernatant;The supernatant of collection, 110000g are centrifuged 70min, abandon supernatant, are resuspended using phosphate buffer Precipitating;110000g is centrifuged 70min again, abandons supernatant, and a small amount of phosphate buffer, which is resuspended, to be precipitated, 0.22 μm of membrane filtration degerming, Obtain source for mesenchymal stem cells exosome.
The exosome in human umbilical cord mesenchymal stem cells source is used to treat the effect assessment of ophthalmology disease model: (1) being regarded Feel electrophysiologic study;(2) clinical observation and scoring;(3) retina pathology section examination;(4) Flow cytometry.
The ophthalmology disease model includes: Mouse Retina damage model, rat experimental autoimmune uvea Retinitis model, Mouse Retina are detached from model.The ophthalmology disease of analog includes: uveitis, detachment of retina, view Retinal damage and inflammation caused by film denaturation and other a variety of causes.
Mould is damaged using the exosome in human umbilical cord mesenchymal stem cells source as drugs local injection Mouse Retina Type, rat experimental autoimmune uveoretinitis model, Mouse Retina are detached from model, it is demonstrated experimentally that exosome With neurotrophy and immunosuppressive action, retinal damage caused by a variety of causes can be mitigated, mitigate inflammatory reaction, thus Improve retinal function, opens up new way for clinical treatment ophthalmology disease.
Possessed by of the invention the utility model has the advantages that
The present invention provides the excretion bodies (exosome) of source for mesenchymal stem cells in preparation treatment ophthalmology disease drug Application.Exosome has neurotrophy and immunosuppressive action, can mitigate retinal damage caused by a variety of causes, subtract Subinflammation reaction opens up new way so as to improve retinal function for clinical treatment ophthalmology disease.
Detailed description of the invention
Exosome is observed under Fig. 1 scanning electron microscope, it is seen that exosome diameter is about 50~100nm, there is complete lipid film, Corpusculum center is in low electron density ingredient, the film property imitated vesicle structure (embodiment 1) of round or ellipse.
Fig. 2 HPLC-MS/MS detects exosome GAP-associated protein GAP: contain 197,180,279 kind of albumen in 3 lot sample sheets respectively, Wherein three samples contain 96 kinds of albumen, including CD9, CD81, Alix, CD44, CD29 (embodiment 1) jointly.
Treatment group and the 1st, 3,7,14,21,40 and 60 day ERG after damage control group mice damage from laser in Fig. 3 embodiment 2 Light a wave and b wave-amplitude.Wherein, A schemes: dark adaptation a wave-amplitude (each time point p value is < 0.05) B figure: dark adaptation b wave Amplitude (each time point p value is < 0.05) C figure: light adaptation a wave-amplitude (the 14th, 21 and 60 day, p value < 0.05) D figure: light adaptation b Wave-amplitude (removes the 3rd beyond the highest heavens, p value is < 0.05).
In Fig. 4 embodiment 2 the 1st after damage from laser, damage control group (A, B, C, D) in 3,7,14 days and treatment group (E, F, G, H) retinal histology slice HE dyeing × 20.1st day visible retina holostrome protuberance, damage location tissue thicken, and structure is disorderly Disorderly.There are defect area, a large amount of inflammatory cell infiltrations in visible outer nuclear layer within 3rd day.7th day visible inner nuclear layer and pigment epithelial layer are thin Born of the same parents migrate to outer nuclear layer.Visible laser spot form tends towards stability within 14th day.Various time points, tissue integrity treatment group are superior to Damage control group.
The statistical result of laser spot parameter measurements in Fig. 5 embodiment 2: laser spot diameter (A) and outer nuclear layer lack completely Damage area's diameter (B) treatment group and damage have statistical difference (p < 0.05) in control group the 3rd, 7 and 14 day.
In Fig. 6 embodiment 2 after damage from laser the 1st, 3,7 and 14 day treatment group and damage control group TUNEL coloration result × 20.4 time point treatment group's apoptotic cells are less than damage control group.
Apoptosis cell statistical result around laser spot in Fig. 7 embodiment 2: it treats within the 1st, 3,7 and 14 day after damage from laser Group is statistically significant (p value is < 0.05) with damage control group apoptosis cell difference.
Different time points exosome treatment group and control group inflammatory reaction clinical score comparison result in Fig. 8 embodiment 3.
Retina paraffin section HE is dyed in Fig. 9 embodiment 3: wherein A, control group the 15th day, shows as inflammatory cell leaching Profit, photoreceptor layer is badly damaged, and each layer has different degrees of denaturation, irregular.B, treatment group the 15th day, retina is not advised Whole lesser extent.C, control group the 21st day, inflammatory cell are reduced, it is seen that photoreceptor damage layer stove.D, treatment group the 21st day, net Film is impaired slight, close to normal.
15th and 21 day histopathological scores after modeling in Figure 10 embodiment 3, from fig. 10 it can be seen that treatment group is significant Lower than model control group.
The expression of immunohistochemistry staining method's detection retina CD68 in Figure 11 embodiment 3: control group the 15th day A, The visible macrophage of a large amount of positive expressions of CD68 invades profit destroying retinal holostrome.B, treatment group the 15th day, CD68 is few in outer nuclear layer Positive expression is measured, retinal structure damage is lighter.C, control group the 21st day, CD68 has a small amount of positive expression in photoreceptor layer. D, treatment group the 21st day, CD68 positive expression is less, and retina is more complete.
The expression of immunohistochemistry staining method's detection retina iNOS in Figure 12 embodiment 3: control group the 15th day A, it can See that each layer of retina especially inner nuclear layer iNOS height is expressed.B, treatment group the 15th day, iNOS expression are less.C, control group the 21st It, is in the still visible positive expression of photoreceptor layer, but it is shallower compared with the 15th day color.D, treatment group the 21st day, iNOS trace expression, Nethike embrane is close to normal.
Flow cytomery control group and exosome treatment group eye CD4+T cell subsets ratio in Figure 13 embodiment 3 Example: CD4+T cell, IFN-γ+CD4+T cell, IL-17+CD4+T cell and Foxp3+CD4+T cell are in ocular cell Ratio.The reduction for the treatment of group's CD4+T cellular infiltration, IFN-γ+CD4+T cell, IL-17+CD4+T cell and Foxp3+CD4+T are thin Born of the same parents' ratio is reduced.
Retinal visual electricity was carried out to each group rat in 12nd day, the 15th day and the 21st day after immune in Figure 14 embodiment 3 Physiological detection, dark adaptation 3.0a wave and b wave treatment group amplitude are apparently higher than control group, statistically significant (a wave t=of difference 3.938,2.726,3.201, P < 0.05, b wave t=8.942,8.161,9.086, P < 0.05).Light adaptation 3.0a wave was at the 15th day Statistically significant (t=5.426,2.463, P < 0.05) with 21 days treatment groups and control group difference, light adaptation 3.0b wave is the 15 days treatment groups and control group difference are statistically significant (t=4.466, P < 0.05)
Treatment group and the 1st, 3,7,14 and 28 day ERG after damage control group mice detachment of retina are dark in Figure 15 embodiment 4 Adapt to a wave and b wave-amplitude.A figure: dark adaptation 0.01a wave-amplitude (each time point p value is < 0.05) B figure: dark adaptation 0.01b wave vibration Width (removes the 28th day, remaining each time point p value is < 0.05) C figure: dark adaptation 3.0a wave-amplitude (removes the 3rd day, remaining each time point p Value < 0.05) D figure: dark adaptation 3.0b wave-amplitude (each time point p value is < 0.05).
The the 1st, 3,7,14,28 day damage control group (A, C, E, G, I) and treatment group after taking off damage are netted in Figure 16 embodiment 4 (B, D, F, H, J) retinal histology is sliced HE dyeing × 20.For 1st day visible nethike embrane holostrome tissue without significant change, RPE layers aobvious It writes and is detached from.The visible de- place's outer nuclear layer oedema of net is obvious within 3rd day, a small amount of inflammatory cell infiltration.7th day visible photoreceptor cell nuclei oedema Mitigate, but inner nuclear layer cell quantity and the number of plies obviously tail off.Visible RPE is attached at neuroepithelial layer again within 14th day, and inflammation is anti- It should almost disappear, tissue morphology tends towards stability.Visible control group outer nuclear layer inner nuclear layer cell arrangement disorder in 28th day, treatment group are each Confluent monolayer cells arrange more neat, Mild edema.Various time points, tissue integrity treatment group are superior to damage control group.
Immunohistochemical staining GFAP:A in Figure 17 embodiment 4, control group the 7th day, GFAP positive expression was in retina Each layer, each layer oedema degree of retina are more serious.B, treatment group the 7th day, GFAP positive expression is substantially reduced compared with control group, each layer Retina structural damage.C, control group the 14th day, a small amount of positive expression of GFAP was in outer nuclear layer, inner nuclear layer.D, treatment group the 14th day, Only minute quantity is expressed in inner nuclear layer, each confluent monolayer cells stable structure to GFAP.
Specific embodiment
The present invention is further explained in the light of specific embodiments.
Embodiment 1:
Human umbilical cord mesenchymal stem cells (human umbilical cordmesenchymal stem cell, hucMSC) The excretion body (exosome) in source isolating and purifying and identifying
1. the isolation and purification method of the excretion body in human umbilical cord mesenchymal stem cells source, includes the following steps:
(1) human umbilical cord mesenchymal stem cells are separately cultured: taking the fresh umbilical cord of sterile newborn, through phosphate buffer (PBS) after repeated flushing, it is cut into the tissue block of diameter about 1-2mm;After 2 Collagenase Types and pancreatin digestion successively, by supernatant Centrifugation, takes cell precipitation to be put into culture bottle, using containing 10% fetal calf serum DMEM/F12 culture medium, 5%CO2, 37 DEG C of saturations it is wet Degree culture;Non-adherent cell is removed, 0.25% trypsin digestion carries out secondary culture after attached cell 80% is merged;
(2) collection of mescenchymal stem cell conditioned medium: the mesenchymal stem cell serum-free culture 48h in 3-5 generation is taken;It receives Collect culture supernatant;0.22 μm of non-velum filteration obtains mescenchymal stem cell conditioned medium;
(3) it includes: 4 DEG C of mescenchymal stem cell conditioned medium for collecting filtering, 1000g centrifugation that exosome, which is isolated and purified, 10min collects supernatant;4 DEG C of the supernatant of collection, 2000g are centrifuged 20min, collect supernatant;4 DEG C of the supernatant of collection, 10000g It is centrifuged 30min, collects supernatant;The supernatant of collection, 110000g are centrifuged 70min, abandon supernatant, are resuspended using phosphate buffer Precipitating;110000g is centrifuged 70min again, abandons supernatant, and a small amount of phosphate buffer, which is resuspended, to be precipitated, 0.22 μm of membrane filtration degerming, Obtain the excretion body (hucMSC-exosome) in human umbilical cord mesenchymal stem cells source.
The identification of 2.hucMSC-exosome
(1) gross morphology of scanning electron microscopic observation exosome: taking the uniform exosome solution of suspension, sample through dehydration, Dry, viscous sample, conductive processing, observe particulate form, and shoot electromicroscopic photograph under scanning electron microscope, randomly select 20 Exosome records its diameter according to scale.It is observed under scanning electron microscope, it is seen that exosome diameter is about 50~100nm, is had complete Lipid film, corpusculum center be in low electron density ingredient, the film property imitated vesicle structure (Fig. 1) of round or ellipse.
(2) HPLC-MS/MS detects exosome GAP-associated protein GAP: 3 lot sample sheets is taken, using high performance liquid chromatography and mass spectrometry The albumen contained in analysis exosome.By the analysis to 3 lot sample sheets, contain 197,180,279 hatching eggs respectively in each sample It is white, wherein three samples contain 96 kinds of albumen jointly, the hucMSC-exosome characteristic protein point such as including CD9, CD81, Alix Son, and with people's umbilical cord derived mesenchymal stem cell marker consistent protein molecular CD44, CD29 (Fig. 2).
Observation of curative effect of the embodiment 2:hucMSC-exosome to Mouse Retina damage model
(1) model foundation: 6~8 SPF grades of week old Healthy female C57BL/6 mouse (15~18g of weight) confirm on inspection to be bent Experiment is included in after light interstitial is clear, eyeground is without exception.Method for breeding is in accordance with Visual and Ophthalmology Research Association about ophthalmology and vision Minimal standards are raised and are used in research.At random by mouse be divided into normal group, treatment group and damage control group.Normal group mouse is not cooked Any processing.Treatment group and damage control group mice are with 500mg/kg dosage 5% chloral hydrate anesthesia of intraperitoneal injection, and right eye is with again After square Tropicamide mydriasis, laser light is carried out using different wavelength krypton lasers machine NOVUS OMNI (Coherent company, the U.S.) Solidifying, laser parameter is as follows: wavelength 647nm, output power 100mW, time for exposure 100ms.Every mouse right eye causes 20 to swash Hot spot more than two away from optic disk disc diameters of each laser spot, between each other apart from least one laser spot diameter, and avoids eye The big blood vessel in bottom.
(2) treatment method and grouping: after damage, treatment group and damage control group mice right eye distinguish intravitreal 5 μ l (0.5mg/ml) hucMSC-exosome and 5 μ l PBS.
(3) evaluation method: the 0th after damage from laser, 2,6,13,20,39 and 59 days, take treatment group and damage control group small Mouse each 6 are put in darkroom overnight, respectively at second day, carry out ERG detection respectively to it.1. dark adaptation ERG: micro- in darkroom Under weak dark red light, 5% chloraldurate intraperitoneal injection of anesthesia, right eye compound tropicamide eye drops mydriasis, 0.4% hydrochloric acid Austria cloth Cacaine eye drops surface anesthesia, 1% sodium carboxymethylcellulose eye drops protect cornea.Mouse prostrate is placed on experimental bench, Filamentary silver annular positive electrode contacts cornea before being placed in right eye, and needle-shaped negative electrode is placed in subcutaneous, needle-shaped ground connection electricity after the pillow between two It is subcutaneous that pole is placed in mouse tail.Photic stimulator provides flash of light, and parameter is as follows: white light, flash time 2.92ms, flash intensity 3.0cd*s/m2, flash of light interval 10s, duplicate measurements 5 times.2. light adaptation ERG: in background luminous intensity 30cd/m2Lower carry out light adaptation 5 minutes.Photic stimulator provides flash of light, and parameter is identical as dark adaptation ERG.Measure a wave, b wave-amplitude.
The the 1st, 3,7 and 14 day after modeling, randomly select normal group mouse 1, treatment group and damage control group mice Each 10, disconnected cervical approach puts to death and wins right side eyeball, and 10% formalin is fixed, conventional to be dehydrated, paraffin embedding.It is cut using tissue Piece machine carries out conventional hematoxylin-Yihong (HE) dyeing through continuously cutting 3 μ m-thicks slice depending on nipple sagittal diameter.Knot of tissue is observed under light microscopic Structure is simultaneously taken pictures, and treatment group and damage control group mice retinal laser spot diameter and outer nuclear layer Defect diameter are measured.
Paraffin section without HE dyeing is multiple through hot repair, be dehydrated and rupture of membranes is handled, the dry sample peripheral region after washing 2 times PBS Domain, according to apoptotic cell dyeing is carried out the step of In situ cell apoptosis detection kit specification, after being incubated for, clean, being dry, DAPI is redyed and mounting.Immediately fluorescence microscopy under the microscope and carry out apoptotic cell counting.
(4) treatment group and damage control group mice ERG dark adaptation and light adaptation a wave, b wave-amplitude are shown in Fig. 3.Dark adaptation a wave Amplitude has statistical difference (t between 7 two groups of time point1=6.865, t2=5.963, t3=2.413, t4=3.794, t5 =2.999, t6=2.475, t7=4.786, p value is < 0.05);Dark adaptation b wave-amplitude has statistical difference 7 time points (t1=3.233, t2=4.019, t3=11.361, t4=6.390, t5=3.612, t6=2.782, t7=2.421, p value < 0.05);There is statistical difference (t within the 14th, 21 and 60 day after injury between two groups of light adaptation a wave-amplitude1=5.711, t2= 2.327 t3=2.786, p < 0.05), the 1st, 3,7 and 40 day a wave-amplitude no significant difference (t between two groups1=1.422, p1=0.181;t2=0.472, p2=0.646;t3=1.772, p3=0.103;t4=2.007, p4=0.069);Light adaptation b Two group difference of wave-amplitude removes the 3rd day (t1=1.753, p1=0.107) statistically significant (t outside1=3.005, t2= 5.238 t3=4.742, t4=5.407, t5=4.029, t6=3.365, p value is < 0.05).
The 1st day after damage from laser, optical microphotograph microscopic observation retina pathological section, it is seen that retina holostrome tissue is grand Rise, pigment epithelial layer cell arrangement disorder, neuroepithelial layer Mild edema, tissue turbulence degree damage control group attach most importance to (Fig. 4 A, 4E).Visible outer nuclear layer injury region is thinning within 3rd day, due to hypochromatosis, outer nuclear layer tissue defect area occurs, also shows inflammation Inflammatory cell infiltration (Fig. 4 B, 4F) in region.Visible outer nuclear layer defect area diameter becomes larger within 7th day, pigment epithelial layer and kernel Confluent monolayer cells fill up defective region to outer nuclear layer migration, and treatment group's cell migration quantity is less than damage control group (Fig. 4 C, 4G).14th day It can be seen that outer nuclear layer defective region is almost filled up by inner nuclear layer and pigment epithelium confluent monolayer cells, inflammatory reaction almost disappears, and tissue morphology becomes In stabilization (Fig. 4 D, 4H).Laser spot diameter treatment group and damage control group the 1st day no difference of science of statistics (t1=1.913, p= 0.071), there are within the 3rd, 7 and 14 day statistical difference (t2=4.697, t3=10.331, t4=5.379, p value is < 0.05) (Fig. 5 A);There is statistical difference in diameter treatment group, outer nuclear layer complete collyriculum area on the 3rd, 7 and 14 day compared with damaging control group (t1=4.176, t2=7.841, t3=6.440, p value is < 0.05) (Fig. 5 B).
The the 1st, 3,7 and 14 day after damage from laser, visible photoreceptor cell nuclei apoptosis (Fig. 6), apoptotic cell quantity treatment group Control group is considerably less than damaged, difference has statistical significance (t1=9.687, t2=7.530, t3=2.094, t4= 3.973, p value is < 0.05) (Fig. 7).
Observation of curative effect of the embodiment 3:hucMSC-exosome to rat experimental autoimmune uveitis model
(1) model foundation: 6~8 week old Female Lewis rats, retinoid binding protein between 30 μ g photoreceptors (IRBP) R16 polypeptide fragment be dissolved in phosphate buffer (PBS) in equal volume containing the complete of 2.5mg/ml tubercle bacillus H37Ra Freund's adjuvant (CFA) mixes in equal volume, and triple valve is fully emulsified.Every rat takes 0.2ml to carry out single metapedes subcutaneous injection and establishes EAU model.
(2) exosome treatment group and model control group treatment method and grouping: are randomly divided into after Lewis rat EAU modeling Each 6.50 μ l of sub-tenon injection capsule contains 30 μ ghucMSC- by every heliosphere since disease initial phase for exosome treatment group The PBS of exosome, continuous injection 7 days, corresponding model control group inject isometric PBS as control.
(3) clinical observation and scoring: start to observe under slit-lamp microscope daily within each group rat 6th day after immune double The performance of ophthalmia disease, scores referring to Caspi clinical scale.Standards of grading are specific as follows: 0 point: no inflammation, eyeground reflection to red light Normally;0.5 point: iris vessels are slightly expanded, are congested;1 point: iris vessels moderate is congested, myosis;2 points: anterior chamber slightly mixes Turbid, eyeground reflection to red light weakens;3 points: anterior chamber's moderate is muddy, and pupil is still as it can be seen that eyeground reflection to red light is dim;4 points: anterior chamber's severe Muddiness, occlusion of pupil, eyeground reflection to red light disappear, proptosis ocular.
Retinal histopathology observation: the 15th day and the 21st day after Lewis rat immunity, eyeball progress is fixed after execution Retinal histopathology HE dyeing, optical microphotograph microscopic observation rat uvea and retina structure, referring to Caspi disease Neo-Confucianism classification is evaluated.
The table of retina immunohistochemistry staining method detection retina CD68 and nitric oxide synthase type (iNOS) It reaches: the 15th day and the 21st day after Lewis rat immunity, eyeball HE stained slice is fixed after execution, uses immunohistochemical staining Method is dyed to Macrophage Surface marker CD68 and mainly by the iNOS of macrophages secrete, optical microphotograph microscopic observation rat Uvea and retina structure.
The detection of retinal visual electro physiology: view was carried out to each group rat in 12nd day, the 15th day and the 21st day after immune The detection of film visual electrophysiology.
Flow cytometer measures Th1, Th17 and Treg cell: the 15th day execution rat after immune takes rat eye and draws Lymph node mononuclearcell is flowed, with flow cytomery Treg cell, Th1 cell and Th17 cell.
(4) clinical score is shown, the 12-16 days, exosome treatment group rat eye clinical score was significantly lower than control Group, difference are statistically significant.(t=3.849,5.121,5.715,6.859,5.830, P < 0.05).(Fig. 8)
Retinal histopathology changes, exosome treatment after retinitis cellular infiltration consistent with clinical manifestation variation Substantially reduced (Fig. 9) is destroyed with institutional framework, each time point (15 days and 21 days) histopathological scores are substantially less than model Control group, difference are statistically significant (Figure 10).(t=4.544,6.708, P < 0.05).
Immunohistochemical staining is shown, the 15th, 21 day after modeling, rat eyes retina CD68 and iNOS positive expression amount It is substantially less than corresponding model control group (Figure 11, Figure 12).
The results show that under inflammatory states, eye CD4+T cellular infiltration increases flow cytomery, with control group phase Than exosome treatment group can reduce CD4+T cell in the ratio of ocular cell, difference statistically significant (t=2.442, P < 0.05), IFN-γ+CD4+T cell, IL-17+CD4+T cell and Foxp3+CD4+T cell lower (t=5.559,4.846, 4.276, P < 0.05) (Figure 13).
The detection of retinal visual electro physiology, detection were carried out to each group rat in 12nd day, the 15th day and the 21st day after immune The a wave and b wave of index dark adaptation and light adaptation 3.0, treatment group's amplitude is obviously higher than control group (Figure 14).
Embodiment 4:hucMSC-exosome is detached from the observation of curative effect of model to Mouse Retina
(1) model foundation: 6~8 SPF grades of week old Healthy female C57BL/6 mouse (15~18g of weight) confirm on inspection to be bent Experiment is included in after light interstitial is clear, eyeground is without exception.Method for breeding is in accordance with Visual and Ophthalmology Research Association about ophthalmology and vision Minimal standards are raised and are used in research.
(2) treatment method and grouping: at random by mouse be divided into normal group, treatment group and damage control group.Normal group mouse It is without any processing.Treatment group and damage control group mice are with 500mg/kg dosage 5% chloral hydrate anesthesia of intraperitoneal injection, right eye After Tropicamide and Phenylephrine mydriasis, artificial detachment of retina is caused using subretinal injection sodium hyaluronate.The dislocation of regulation net is set Above temporo side or temporo, de- area about 30%-40% is netted, the animal mould for not meeting the above standard and haveing damage bleeding is cast out Type.After damage, treatment group and damage control group mice right eye distinguish intravitreal 5 μ l (0.5mg/ml) hucMSC- Exosome and 5 μ l PBS.
(3) evaluation method: the 1st after modeling, 3,7,14,28 days, treatment group and damage control group mice each 6 is taken to be put in In darkroom overnight, respectively at second day, ERG detection is carried out respectively to it.Dark adaptation ERG: in darkroom under faint dark red light, 5% chloraldurate intraperitoneal injection of anesthesia, right eye compound tropicamide eye drops mydriasis, 0.4% Oxybuprocaine hydrochloride eye drops Surface anesthesia, 1% sodium carboxymethylcellulose eye drops protect cornea.Mouse prostrate is placed on experimental bench, filamentary silver annular is just Electrode contacts cornea before being placed in right eye, and needle-shaped negative electrode is placed in after the pillow between two subcutaneously, and needle-shaped grounding electrode is placed in mouse Tail portion is subcutaneous.Photic stimulator provides flash of light, and parameter is as follows: white light, flash time 2.92ms, flash intensity 3.0cd*s/m2, dodge Light interval 10s, duplicate measurements 5 times.Measure a wave, b wave-amplitude.
The the 1st, 3,7,14 and 28 day after modeling, normal group mouse 1 is randomly selected, treatment group and damage control group are small Mouse each 10, disconnected cervical approach puts to death and wins right side eyeball, and 10% formalin is fixed, conventional to be dehydrated, paraffin embedding.Using tissue Slicer carries out conventional hematoxylin-Yihong (HE) dyeing and immunohistochemical staining through continuously cutting 3 μ m-thicks slice depending on nipple sagittal diameter. Institutional framework is observed under light microscopic and is taken pictures.
(4) treatment group and damage control group mice ERG dark adaptation a wave, b wave-amplitude are shown in Figure 15.Dark adaptation 0.01a wave-amplitude There is statistical difference (t between 5 two groups of time point1=3.334, t2=3.814, t3=3.961, t4=6.645, t5= 8.793, p value is < 0.05);Beyond the highest heavens except the 28th, various time points have statistics poor to two groups of differences of dark adaptation 0.01b wave-amplitude Different (t1=5.131, t2=8.091, t3=4.335, t4=2.213, p value is < 0.05);Two groups of dark adaptation 3.0a wave-amplitude is poor Different to remove the 3rd beyond the highest heavens, various time points have statistical difference (t1=2.898, t2=2.665, t3=3.958, t4=3.876, p <0.05);Statistically significant (t between two groups of dark adaptation 3.0b wave-amplitude1=7.953, t2=4.976, t3=6.069, t4= 2.639 t5=9.859, p value is < 0.05).
The 1st day after the de- damage of net, optical microphotograph microscopic observation retina pathological section, it is seen that retina holostrome tissue is without bright Aobvious variation, RPE layers of significant disengaging, neuroepithelial layer Mild edema, tissue turbulence degree damage control group and treatment group without obvious Difference (Figure 16 A, 16B).The visible de- place's outer nuclear layer oedema of net is obvious within 3rd day, also shows a small amount of inflammatory cell leaching in areas of inflammation Profit, damage control group are more obvious compared with treatment group's oedema degree (Figure 16 C, 16D).Visible photoreceptor cell nuclei oedema mitigates within 7th day, But inner nuclear layer cell quantity and the number of plies obviously tail off, and ganglion-cell layer oedema mitigates, outer nuclear layer and inner nuclear layer cell arrangement pair According to group compared with treatment group's more disorder (Figure 16 E, 16F).Visible treatment group RPE is attached at neuroepithelial layer, inflammation again within 14th day Reaction almost disappears, and tissue morphology tends towards stability (Figure 16 G, 16H).28th day visible control group outer nuclear layer inner nuclear layer cell arrangement Disorder, each confluent monolayer cells for the treatment of group arrange more neat, Mild edema (Figure 16 I, 16J).
Immunohistochemical staining is shown, 7th, 14 day after modeling net is de-, treatment group's rat eyes retina GFAP positive table Model control group is substantially less than up to amount.(Figure 17)
It is above-mentioned small as drugs local injection using the exosome in human umbilical cord mesenchymal stem cells source of the present invention Rat retina damage model, rat experimental autoimmune uveoretinitis model, Mouse Retina are detached from model It is demonstrated experimentally that exosome have neurotrophy and immunosuppressive action, can mitigate retinal damage caused by a variety of causes, Mitigate inflammatory reaction, so as to improve retinal function, opens up new way for clinical treatment ophthalmology disease.

Claims (1)

1. application of the excretion body of source for mesenchymal stem cells in preparation treatment ophthalmology disease drug, the mesenchyma are dry thin Born of the same parents be people's umbilical cord source mescenchymal stem cell, the ophthalmology disease be Autoimmune uveitis disease, retinal damage, Detachment of retina.
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